Redox electrodeposition polymers: adaptation of the redox potential of polymer-bound Os complexes for bioanalytical applications

The design of polymers carrying suitable ligands for coordinating Os complexes in ligand exchange reactions against labile chloro ligands is a strategy for the synthesis of redox polymers with bound Os centers which exhibit a wide variation in their redox potential. This strategy is applied to polymers with an additional variation of the properties of the polymer backbone with respect to pH-dependent solubility, monomer composition, hydrophilicity etc. A library of Os-complex-modified electrodeposition polymers was synthesized and initially tested with respect to their electron-transfer ability in combination with enzymes such as glucose oxidase, cellobiose dehydrogenase, and PQQ-dependent glucose dehydrogenase entrapped during the pH-induced deposition process. The different polymer-bound Os complexes in a library containing 50 different redox polymers allowed the statistical evaluation of the impact of an individual ligand to the overall redox potential of an Os complex. Using a simple linear regression algorithm prediction of the redox potential of Os complexes becomes feasible. Thus, a redox polymer can now be designed to optimally interact in electron-transfer reactions with a selected enzyme.     

Conducting Redoxpolymer-Based Reagentless Biosensors Using Modified PQQ-Dependent Glucose Dehydrogenase

Reagentless, oxygen-independent glucose biosensors based on an Os-complex-modified polypyrrole matrix and on soluble PQQ-dependent glucose dehydrogenase from Acinetobacter calcoaceticus are described.As the soluble form of glucose dehydrogenase from Acinetobacter calcoaceticus is a hydrophilic enzyme with a positive net charge, its entrapment into the positively charged hydrophobic polypyrrole film is much more complicated than that of the corresponding membrane enzyme or the negatively charged and very stable glucose oxidase. Possible ways for using soluble PQQ-dependent glucose dehydrogenase in combination with conducting polymer films are seen in the modulation of the enzyme properties by covalent binding of suitable compounds to the protein shell together with the adjustment of the properties of the conducting polymer film. This can be done by neutralising the net charge of the protein and/or optimising the electron-transfer pathway between enzyme and electrode surface by covalent binding of suitable redox relays to the protein surface.In addition, methods for increasing the hydrophilicity of the polymer film, such as the co-entrapment of high-molecular weight hydrophilic additives and copolymerisation of hydrophilic pyrrole derivatives are presented. It is demonstrated that the replacement of the parent monomer pyrrole by a suitable hydrophilic pyrrole derivative facilitates the entrapment of the modified soluble PQQ-dependent glucose dehydrogenase into the Os-complex-modified polymer and hence allows for the development of reagentless biosensors.     

Design of an Os Complex‐Modified Hydrogel with Optimized Redox Potential for Biosensors and Biofuel Cells

Multistep synthesis and electrochemical characterization of an Os complex‐modified redox hydrogel exhibiting a redox potential ≈+30 mV (vs. Ag/AgCl 3 m KCl) is demonstrated. The careful selection of bipyridine‐based ligands bearing N,N‐dimethylamino moieties and an amino‐linker for the covalent attachment to the polymer backbone ensures the formation of a stable redox polymer with an envisaged redox potential close to 0 V. Most importantly, the formation of an octahedral N6‐coordination sphere around the Os central atoms provides improved stability concomitantly with the low formal potential, a low reorganization energy during the Os^3+/2+ redox conversion and a negligible impact on oxygen reduction. By wiring a variety of enzymes such as pyrroloquinoline quinone (PQQ)‐dependent glucose dehydrogenase, flavin adenine dinucleotide (FAD)‐dependent glucose dehydrogenase and the FAD‐dependent dehydrogenase domain of cellobiose dehydrogenase, low‐potential glucose biosensors could be obtained with negligible co‐oxidation of common interfering compounds such as uric acid or ascorbic acid. In combination with a bilirubin oxidase‐based biocathode, enzymatic biofuel cells with open‐circuit voltages of up to 0.54 V were obtained.     

A new self-assembled modified electrode for competitive immunoassay

Alternating films constructed upon successive deposition of redox polymer Os(bpy)₂ClPyCH₂NHpoly(allylamine) and antibiotin IgG were developed for amperometric immunosensor design. Cyclic voltammetric measurements were used to verify charge transport between redox sites and the redox surface concentration was estimated upon voltammetric peak integration. Biotin–antibiotin complex formation was evaluated using horseradish peroxidase as an enzyme label. Redox mediation between the modified electrode surface and the redox site in the enzyme was verified after substrate addition. Multilayer modified gold electrodes with biologically active antibiotin IgG molecules were employed for the development of a competitive immunoassay with electrochemical label detection.     

Microstructural and Potential Dependence Studies of Urease-Immobilized Gold Nanoparticles–Polypyrrole Composite Film for Urea Detection

Gold nanoparticle–polypyrrole nanocomposite film was electrochemically deposited in a single-step polymerization of pyrrole in the presence of 3-mercaptopropionic acid (MPA)-capped gold nanoparticles (GNPs) and p-toluenesulfonic acid (pTSA) on the surface of an indium tin oxide (ITO)-coated glass plate. The carboxyl functional groups surrounding the GNPs within the polymer matrix were utilized for the immobilization of urease enzyme through carbodiimide coupling reaction for the construction of a Urs/GNP(MPA)–PPy/ITO-glass bioelectrode for urea detection in Tris–HCl buffer. The resulting bioelectrode film was characterized by atomic force microscopy (AFM), high-resolution transmission electron microscopy (HRTEM), contact angle measurement, Fourier transform infrared spectroscopy (FTIR), and electrochemical techniques. The potentiometric response of the bioelectrode made of polymer nanocomposite films of two different thicknesses prepared at 100 and 250 mC cm^?2 charge densities, respectively, was studied towards the urea concentration in Tris–HCl buffer (pH 7.4). The thin polymer nanocomposite film-based bioelectrode prepared at 100 mC cm^?2 charge density exhibited a comparatively good potentiometric response than a thick 250 mC cm^?2 charge density film with a linear range of urea detection from 0.01 to 10 mM with a sensitivity of 29.7 mV per decade.     

Enzyme activity control by responsive redoxpolymers

A new thermoresponsive poly-N-isopropylacrylamide (PNIPAM)-ferrocene polymer was synthesized and characterized. PNIPAMFoxy bears additional oxirane groups which were used for attachment by a self-assembly process on a cysteamine-modified gold electrode to create a thin hydrophilic film. The new redox polymer enabled electrical communication between the cofactor pyrrolinoquinoline quinone (PQQ) of soluble glucose dehydrogenase (sGDH) and the electrode for sensitive detection of this enzyme as a prospective protein label. The temperature influence on the redox polymer/enzyme complex was investigated. An inverse temperature response behavior of surface bound PNIPAMFoxy compared to the soluble polymer was found and is discussed in detail. The highest efficiency of mediated electron transfer for the immobilized PNIPAMFoxy with sGDH was observed at 24 degrees C, which was twice as high as that of its soluble counterpart. A steady-state electrooxidation current densitiy of 4.5 microA.cm-2 was observed in the presence of 10 nM sGDH and 5 mM glucose. A detection limit of 0.5 nM of soluble PQQ-sGDH was obtained.     

Evaluation of osmium(II) complexes as electron transfer mediators accessible for amperometric glucose sensors.

In order to lower the redox potentials of Os(III/II) complexes, the mixed ligand complexes of Os(II) were synthesized. The redox potentials of Os(III/II) complexes could be lowered by the use of 4,4'-dimethyl-2,2'-bipyridine (dmbpy), imidazole (Him) or its derivatives, and chloride ion as ligands, e.g., values of the redox (formal) potentials of 628 mV vs. Ag/AgCl for [Os(bpy)3]3+/2+ (bpy: 2,2'-bipyridine) and -6 mV for [OsCl(Him)(dmbpy)2]2+/+ were given in deaerated 0.1 mol dm-3 phosphate buffer (pH 7.0). The evaluation of Os(II) complexes as electron transfer mediators accessible for amperometric glucose sensors was examined according to the determination of the redox potentials of Os(III/II) complexes and the second-order rate constants for electron transfer between glucose oxidase (GOx) in reduced form and the Os(III) complex. Although the Os(II) complexes with lower redox potentials tended to decrease the second-order rate constants ks, the ks values for the majority of Os(II) complexes synthesized in this study were greater than that for ferrocenecarboxylic acid. Acceleration of the electron-transfer reaction is attributable to the hydrogen bonding and/or the electrostatic interaction between the Os(II) complexes and GOx. It may be consequently concluded that the mixed ligand complexes of Os(II) with bpy (dmbpy), Him (its derivatives), and Cl- can act as more efficient electron transfer mediators for the fabrication of amperometric glucose sensors.     

Augmentation of enzyme electrode sensitivity using biocatalytic preconcentration

A method for increasing the sensitivity of enzyme sensors based on biocatalytic accumulation of an intermediate product was investigated using a biospecific electrode consisting of an immobilized glucose dehydrogenase-lactate dehydrogenase-lactate monooxygenase membrane and an electrochemical oxygen probe. Addition of the analyte (glucose) and an excess of NAD⁺ to the background solution permits NADH to be biocatalytically preconcentrated in the enzyme membrane. When this reaction has approached equilibrium, the sensor signal is generated by injection of an excess of pyruvate, thus starting oxygen consumption catalysed by the sequential lactate dehydrogenase-lactate monooxygenase reaction. Glucose can be determined at concentrations between 10 and 100 μM. Compared with operation of the sensor without NADH preconcentration, the increase in the sensitivity to glucose is 18-fold in the current-time mode and 40-fold in the derivative current-time mode. The measuring regime permits interferences from the sample solution to be avoided.     

Long tethers binding redox centers to polymer backbones enhance electron transport in enzyme "Wiring" hydrogels

A redox hydrogel with an apparent electron diffusion coefficient (D(app)) of (5.8 +/- 0.5) x 10(-)(6) cm(2) s(-)(1) is described. The order of magnitude increase in D(app) relative to previously studied redox hydrogels results from the tethering of redox centers to the backbone of the cross-linked redox polymer backbone through 13 atom spacer arms. The long and flexible tethers allow the redox centers to sweep electrons from large-volume elements and to collect electrons of glucose oxidase efficiently. The spacer arms make the collection of electrons from glucose oxidase so efficient that glucose is electrooxidized already at -0.36 V versus Ag/AgCl, the reversible potential of the redox potential of the FAD/FADH(2) centers of the enzyme at pH 7.2. The limiting current density of 1.15 mA cm(-)(2) is reached at a potential as low as -0.1 V versus Ag/AgCl. The novel redox center of the polymer is a tris-dialkylated N,N'-biimidazole Os(2+/3+) complex. Its redox potential, -0.195 V versus Ag/AgCl, is 0.8 V reducing relative to that of Os(bpy)(2+/3+), its 2,2'-bipyridine analogue.     

Fabrication of a Highly Sensitive Glucose Biosensor Based on Immobilization of Osmium Complex and Glucose Oxidase onto Carbon Nanotubes Modified Electrode

In this research a novel osmium complex was used as electrocatalyst for electroreduction of oxygen and H₂O₂ in physiological pH solutions. Electroless deposition at a short period of time (60 s), was used for strong and irreversible adsorption of 1,4,8,12‐tetraazacyclotetradecane osmium(III) chloride (Os(III)LCl₂) ClO₄ onto single‐walled carbon nanotubes (SWCNTs) modified GC electrode. The modified electrode shows a pair of well defined and reversible redox couple, Os(IV)/Os(III) at wide pH range (1–8). The glucose biosensor was fabricated by covering a thin film of glucose oxidase onto CNTs/Os‐complex modified electrode. The biosensor can be used successfully for selective detection of glucose based on the decreasing of cathodic peak current of oxygen. The fabricated biosensor shows high sensitivity, 826.3 nA μM^?1cm^?2, low detection limit, 56 nM, fast response time <3 s and wide calibration range 1.0 μM–1.0 mM. The biosensor has been successfully applied to determination of glucose in human plasma. Because of relative low applied potential, the interference from electroactive existing species was minimized, which improved the selectivity of the biosensor. The apparent Michaelis‐Menten constant of GOx on the nanocomposite, 0.91 mM, exhibits excellent bioelectrocatalytic activity of immobilized enzyme toward glucose oxidation. Excellent electrochemical reversibility, high stability, technically simple and possibility of preparation at short period of time are of great advantages of this glucose biosensor.     

A Carbon Nanotube Layered Electrode for the Construction of the Wired Bilirubin Oxidase Oxygen Cathode

Oxidatively treated carbon nanotubes were coated on a glassy carbon surface to form a CNT‐layer. On the CNT‐layered GC surface, a redox hydrogel film of the copolymer, of polyacryamide and poly(N‐vinylimidazole) complexed with [Os(4,4′‐dichloro‐2,2′‐bipyridine)₂Cl]^+/2+ wiring bilirubin oxidase was immobilized. A good contact was achieved between the hydrogel film and the hydrophilic CNT‐layer with carboxylated CNTs. The prepared bilirubin oxidase cathode on the CNT‐layer was employed for the electrocatalytic reduction of O₂, and enhanced current and stability were observed. Electron transfers from the electrode surface O₂ molecules were analyzed. The optimal composition of the enzyme, redox polymer, and cross‐linker in the catalyst and the thickness of the CNT‐layer were determined.     

Glucose nanosensors based on redox polymer/glucose oxidase modified carbon fiber nanoelectrodes

This paper describes glucose nanosensors based on the co-electrodeposition of a poly(vinylimidazole) complex of [Os(bpy)₂Cl]^+/2+ and glucose oxidase (GOD) on a low-noise carbon fiber nanoelectrodes (CFNE). The SEM image shows that the osmium redox polymer/enzyme composite film is uniform. The film modified CFNE exhibits the classical features of a kinetically fast redox couple bound to the electrode surface. A strong and stable electrocatalytic current is observed in the presence of glucose. Under the optimal experimental conditions, the nanosensor offers a highly sensitive and rapid response to glucose at an operating potential of 0.22 V. A wide linear dynamic rang of 0.01-15 mM range was achieved with a detection limit of 0.004 mM. Compared with the conventional gold electrode, the nanosensor possessed higher sensitivity and longer stability. Successful attempts were made in real time monitoring rabbit blood glucose levels.     

Specific and Rapid Glucose Detection Using NAD‐dependent Glucose Dehydrogenase,Diaphorase, and Osmium Complex

Selective glucose measurement in serum and blood and rapid glucose measurement using nicotinamide adenine dinucleotide (NAD)‐dependent glucose dehydrogenase (NAD‐GDH) are still very challenging. Here, we report a selective and rapid glucose sensor, based on electrochemical‐enzymatic‐enzymatic (ENN) redox cycling involving bis(2,2‐bipyridyl)dichloroosmium(II) [Os(bpy)₂Cl₂], diaphorase (DI), NAD⁺, NAD‐GDH, and glucose. DI and Os(bpy)₂Cl₂ are used to obtain fast mediated oxidation of NADH that is generated as a result of glucose oxidation by NAD‐GDH. DI and NAD‐GDH are co‐immobilized via affinity binding on an avidin‐modified indium tin oxide electrode to obtain fast and stable ENN redox cycling. Two enzymes (DI and NAD‐GDH) and two electron mediators [Os(bpy)₂Cl₂ and NAD⁺] are insensitive to oxygen. The applied potential (0.0 V vs Ag/AgCl) is low enough to minimize interfering electrochemical reactions, and the redox reactions of Os(bpy)₂Cl₂ with interfering species are slow. NAD‐GDH is much less reactive to problematic monosaccharides such as xylose, fructose, galactose, and mannose than glucose. Artificial serum containing 5 % (w/v) human serum albumin shows a similar electrochemical background level in serum. All results enable us to obtain selective and reproducible glucose detection. The fast ENN redox cycling allows sensitive glucose detection with a wide range of concentrations in artificial serum with a short measuring time (5 s) without an incubation period.     

Quinoprotein glucose dehydrogenase modified thick-film electrodes for the amperometric detection of phenolic compounds in flow injection analysis

The use of thick-film electrodes as basic transducers for highly sensitive amperometric biosensors using PQQ (pyrroloquinoline quinone) dependent glucose dehydrogenase (GDH) with short response times is described. The enzyme is embedded in a polyurethane matrix on top of a platinum based thick film electrode and its ability to reduce oxidized phenolic compounds is exploited. The electrochemical amplification is based on the oxidation of the analyte on the surface of the electrode followed by its enzymatic reduction. Different parameters of the glucose dehydrogenase electrode system using dopamine as a model analyte were optimized, e.g., membrane thickness, pH value, buffer system, flow rate and storage conditions. Using optimized parameters the sensitivity and detection limits for various phenolic compounds were evaluated. The comparison of electrodes from the identical as well as from different batches shows the ability to produce a number of well reproducible sensors showing remarkably small differences with respect to parameters as sensitivity, response times and measuring range.     

Synthesis and Electrochemical Characterization of a New Electropolymerizable Hydrophilic Viologen Designed for Enzyme Wiring

A new viologen derivative functionalized by an electropolymerizable pyrrole group via a long hydrophilic spacer has been synthesized. This redox monomer has been electrochemically characterized both for its presence in organic and in aqueous media. Its electrooxidation in both solvents leads to the formation of a polymeric film exhibiting the regular electrochemical behaviour of the viologen groups. The electropolymerization process was applied to the immobilization of isocitrate dehydrogenase as an enzyme model. An electrical connection between the redox polymer and the immobilized enzyme molecules has been observed in the presence of oxoglutarate and CO₂.     

Analytical Characteristics of Electrochemical Biosensor Using Pt‐Dispersed Graphene on Boron Doped Diamond Electrode

An electrochemical biosensor was developed using Pt‐nanoparticles (Pt‐NPs) dispersed graphene based on a boron‐doped diamond thin film electrode. To compare its performances with those of other biosensors, glucose was used as a target analyte. This biosensor exhibited a wide linear range, a low detection limit and a higher sensitivity compared to other amperometric biosensors using graphene‐based electrodes. In addition, the biosensor promotes a direct electron transfer between the redox enzymes and the electrode surface and detects low concentration analytes. The excellent performance of the biosensor is attributed to the synergistic effect of the Pt‐NPs, graphene sheet and the BDD thin film. Therefore, it can be a promising application for electrochemical detection of analytes.     

Effect of Gold Nanoparticles on the Structure and Electron‐Transfer Characteristics of Glucose Oxidase Redox Polyelectrolyte‐Surfactant Complexes

Efficient electrical communication between redox proteins and electrodes is a critical issue in the operation and development of amperometric biosensors. The present study explores the advantages of a nanostructured redox‐active polyelectrolyte–surfactant complex containing [Os(bpy)₂Clpy]²⁺ (bpy=2,2′‐bipyridine, py= pyridine) as the redox centers and gold nanoparticles (AuNPs) as nanodomains for boosting the electron‐transfer propagation throughout the assembled film in the presence of glucose oxidase (GOx). Film structure was characterized by grazing‐incidence small‐angle X‐ray scattering (GISAXS) and atomic force microscopy (AFM), GOx incorporation was followed by surface plasmon resonance (SPR) and quartz‐crystal microbalance with dissipation (QCM‐D), whereas Raman spectroelectrochemistry and electrochemical studies confirmed the ability of the entrapped gold nanoparticles to enhance the electron‐transfer processes between the enzyme and the electrode surface. Our results show that nanocomposite films exhibit five‐fold increase in current response to glucose compared with analogous supramolecular AuNP‐free films. The introduction of colloidal gold promotes drastic mesostructural changes in the film, which in turn leads to a rigid, amorphous interfacial architecture where nanoparticles, redox centers, and GOx remain in close proximity, thus improving the electron‐transfer process.     

Quinoprotein glucose dehydrogenase modified thick-film electrodes for the amperometric detection of phenolic compounds in flow injection analysis

The use of thick-film electrodes as basic transducers for highly sensitive amperometric biosensors using PQQ (pyrroloquinoline quinone) dependent glucose dehydrogenase (GDH) with short response times is described. The enzyme is embedded in a polyurethane matrix on top of a platinum based thick film electrode and its ability to reduce oxidized phenolic compounds is exploited. The electrochemical amplification is based on the oxidation of the analyte on the surface of the electrode followed by its enzymatic reduction. Different parameters of the glucose dehydrogenase electrode system using dopamine as a model analyte were optimized, e.g., membrane thickness, pH value, buffer system, flow rate and storage conditions. Using optimized parameters the sensitivity and detection limits for various phenolic compounds were evaluated. The comparison of electrodes from the identical as well as from different batches shows the ability to produce a number of well reproducible sensors showing remarkably small differences with respect to parameters as sensitivity, response times, and measuring range. Received: 15 August 2000 / Revised: 17 October 2000 / Accepted: 24 October 2000     

Coupled enzyme reaction microarrays based on pin-printing of sol–gel derived biomaterials

We report on the development of a new class of protein microarrays based on the co-immobilization of multiple components within a single pin-printed sol–gel array element. In the first case, the microarraying of a coupled two enzyme reaction involving glucose oxidase and horseradish peroxidase along with the fluorogenic reagent Amplex Red is demonstrated to allow “reagentless” fluorimetric detection of glucose. The second system involved the detection of urea using co-immobilized urease and fluorescein dextran, which works on the basis of a pH induced change in fluorescein emission intensity upon production of ammonium carbonate owing to hydrolysis of urea. In both the cases, it is demonstrated that the changes in intensity from the array are time-dependent, consistent with the enzyme catalyzed reaction, showing that such arrays can be used for kinetic studies. The rate of intensity change was also found to be dependent on the concentration of analyte added to the array, showing that such arrays could be useful for quantitative multianalyte biosensing. Inhibition of urease by the competitive inhibitor thiourea is also demonstrated on a microarray, demonstrating that sol–gel-based microarrays may find use in high-throughput drug-screening applications.     

Electrolyte effects on electrochemical properties of osmium complex polymer modified electrodes.

The electrolyte effects on the electrochemical behaviors of osmium complex polymer modified electrodes were investigated by a comparison between two osmium complexes, [Os(bpy)2(PVI)10Cl]Cl (Os-PVI10) and [Os(bpy)2(PVP)10Cl]Cl (Os-PVP10). The electrode process at Os-PVI10 modified electrodes is reaction-controlled, while a diffusion-controlled electrode process exists at Os-PVP10 modified electrodes. Both the cation and anion in supporting electrolytes strongly affect their electrochemical behaviors, such as the redox potential, wave shape and peak current. These phenomena are attributed to a change in the film structure and polymer swelling in various supporting electrolytes. The influence of electrolyte anions on the electrochemical behaviors is related to their hydrophobicity. The electrode process of Os-PVP10 depends on the pH value of solutions, exhibiting different electron transfer mechanisms.